Lead Optimization of Imidazopyrazines: A New Class of Antimalarial

Department of Pediatrics, School of Medicine, University of California, San Diego, California 92093, United States. ACS Med. ... Journal of Medicinal ...
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Lead Optimization of Imidazopyrazines: A New Class of Antimalarial with Activity on Plasmodium Liver Stages Bin Zou,*,† Advait Nagle,‡ Arnab K. Chatterjee,‡ Seh Yong Leong,† Liying Jocelyn Tan,† Wei Lin Sandra Sim,† Pranab Mishra,‡ Prasuna Guntapalli,‡ David C. Tully,‡ Suresh B. Lakshminarayana,† Chek Shik Lim,† Yong Cheng Tan,† Siti Nurdiana Abas,† Christophe Bodenreider,† Kelli L. Kuhen,‡ Kerstin Gagaring,‡ Rachel Borboa,‡ Jonathan Chang,‡ Chun Li,‡ Thomas Hollenbeck,‡ Tove Tuntland,‡ Anne-Marie Zeeman,§ Clemens H. M. Kocken,§ Case McNamara,‡ Nobutaka Kato,‡ Elizabeth A. Winzeler,‡,∥ Bryan K. S. Yeung,† Thierry T. Diagana,† Paul W. Smith,† and Jason Roland*,‡ †

Novartis Institute for Tropical Diseases, 10 Biopolis Road #05-01 Chromos, 138670 Singapore Genomics Institute of the Novartis Research Foundation, San Diego, California 92121, United States § Department of Parasitology, Biomedical Primate Research Centre, 2280 GH Rijswijk, The Netherlands ∥ Department of Pediatrics, School of Medicine, University of California, San Diego, California 92093, United States ‡

S Supporting Information *

ABSTRACT: Imidazopyridine 1 was identified from a phenotypic screen against P. falciparum (Pf) blood stages and subsequently optimized for activity on liver-stage schizonts of the rodent parasite P. yoelii (Py) as well as hypnozoites of the simian parasite P. cynomolgi (Pc). We applied these various assays to the cell-based lead optimization of the imidazopyrazines, exemplified by 3 (KAI407), and show that optimized compounds within the series with improved pharmacokinetic properties achieve causal prophylactic activity in vivo and may have the potential to target the dormant stages of P. vivax malaria. KEYWORDS: Liver-stage antimalarial, imidazopyrazines, structure−activity relationship, lead optimization

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subsequent candidate with optimal drug-like properties could then be evaluated in the P. cynomolgi infected monkey model as a test for radical cure activity.11 From a previous phenotypic screening effort on Pf blood stages, we selected imidazopyridine 1 as a starting point despite its relatively weak activity (Figure 1).12 Early hit-to-lead chemistry on the two distal aromatic rings resulted in the identification of 2, a compound that showed a greater than 50fold increase in potency. Although compound 2 was active on blood stages, it was still relatively inactive on Py schizonts and Pc and suffered from poor physicochemical properties, presumably due to the high lipophilicity (cLogP = 4.3). Modification of the bicyclic core by installation of a nitrogen atom at the 7 position reduced the cLogP by one log unit and resulted in 3 (KAI407).8 Although the potency on Pf blood stages was diminished, incorporating the imidazolopyrazine core resulted in a compound with improved activity on Py and Pc liver stages.

alaria continues to be a significant public health problem, threatening up to 40% of the global population.1 Among the five species of malaria parasites that infect humans,2 P. vivax malaria alone causes approximately 80−300 million clinical cases annually.3−5 Primaquine, the only licensed drug for the radical cure of P. vivax, is contraindicated in glucose-6-phosphate dehydrogenase (G6PD)-deficient populations,6 and the recommended long-term treatment (30 mg/ kg for 14 days) precludes its widespread use. Thus, there remains an urgent need to develop non-8-aminoquinolines as safe and effective therapeutics for radical cure of P. vivax. From a drug discovery perspective, finding potential radical curative agents requires identifying compounds that also target the liver stages of the parasite. We recently described two in vitro assays, which can identify compounds targeting developing schizonts and quiescent hypnozoites in hepatocytes.7−9 These assays utilize the rodent P. yoelii (Py) and the simian P. cynomolgi (Pc) parasites to target the liver schizonts and hypnozoites, respectively.10 We sought to develop a screening strategy involving both bloodand liver-stage assays to identify compounds with biological activity on multiple parasite life stages with the ultimate goal of developing radical curative agent for P. vivax malaria. A © XXXX American Chemical Society

Received: June 9, 2014 Accepted: July 6, 2014

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dx.doi.org/10.1021/ml500244m | ACS Med. Chem. Lett. XXXX, XXX, XXX−XXX

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imidazopyrazine core (6).13 A regioselective bromination at C3 with NBS provided 3-bromo-6-carboxylate 7 as the sole product isolated.14 Hydrolysis of 7 to the corresponding acid (8) followed by amide bond formation with an appropriate amine provided compound 9. Finally, Suzuki coupling with a series of boronic acids yielded the corresponding imidazopyrazine analogues.15 As we explored the SAR around the R1 position of the imidazopyrazine core, we found that para-substituted N-phenyl or N-pyridyl were favored, while other heterocycles such as pyridazine (12) or benzothiazole (13) resulted in a loss of activity on both blood and liver stages (Table 1). In addition, the benzyl derivative (14), or replacement with a piperidine Table 1. Blood- and Liver-Stage (Schizont) Activity of the Imidazopyrazinesa

Figure 1. In vitro activity of compounds 1−3 on multiple parasite life stages.

The added activity of compound 3 on Py schizonts and Pc hypnozoites suggested that changes to the bicyclic core could impart the desired liver-stage activity to the molecule. We further hypothesized that activity in the Py assay might be predictive of potency on Pc hypnozoites for this chemical class and could therefore be used as a first-pass screen due to the low throughput of the Pc assay. Following the discovery of compound 3, we initiated a lead optimization effort in an attempt to identify a compound with an optimal potency and PK profile. The overall strategy focused on making peripheral changes around the bicyclic imidazopyrazine core. This feature, along with the C3 phenyl and amide linker was found to be the main pharmacophore responsible for activity on Pc hypnozoites in vitro. Thus, analogues could be prepared from a primary building block consisting of the imidazopyrazine core (8) and chemically elaborated to 10−20 (Scheme 1). Briefly, 2-chloroacetaldehyde 5 was added to a solution of aminopyrazine 4 in ethanol and heated to reflux to afford the Scheme 1. Synthetic Route to the Imidazopyrazinesa

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Reagents and conditions: (a) 2-chloroacetaldehyde 5 (50 wt % solution in water), NaHCO 3, ethanol, reflux, 70%; (b) Nbromosuccinimide (NBS), CH2Cl2, room temperature (rt), 94%; (c) NaOH, THF/H2O, 60 °C, 56%; (d) oxalyl dichloride, CH2Cl2, DMF (a drop), 30 min, followed by amine, rt; (e) boronic acid, Pd(PPh3)4 (5−10 mol %), aqueous KF solution (2 M), microwave, 110 °C, 30 min to 1 h.

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IC50 values are the average of at least two independent experiments. dx.doi.org/10.1021/ml500244m | ACS Med. Chem. Lett. XXXX, XXX, XXX−XXX

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the improved solubility would translate to a better in vivo PK profile, compounds 17−20 were evaluated in mice by oral (p.o.) and intravenous (i.v.) routes at 20 and 5 mg/kg, respectively (Table 4). Of the four compounds evaluated, 18 and 19 were more soluble and displayed favorable PK properties with moderate clearance, low volume of distribution, and moderate bioavailability (∼50%). Increasing the clogP slightly by alkylating the primary carboxamide (20) further boosted Cmax and exposure levels while lowering clearance and increasing the bioavailability (60%). If Py liver schizonts are being inhibited in vitro, then the assay should predict that active compounds with an acceptable pharmacokinetic profile display causal prophylactic activity in vivo by preventing the parasite from establishing itself in the liver. In order to evaluate the in vivo efficacy of this class of compounds, analogues 3 and 18−20 were tested in a causal prophylaxis P. berghei mouse model (Figure 2). When

ring (15), resulted in a loss of potency suggesting a narrow range of tolerated substitutions at the R1-position. The C3 phenyl was an essential part of the pharmacophore, and parasubstitutions were preferred. Optimization of the R2 groups revealed the carboxamide as the optimal substituent, providing, a good balance between potency and physicochemical properties (18−20). Other R2 substituents such as dimethylamine, methylsulfones, and carboxylic acids were inactive (data not shown). Interestingly adding an additional heterocycle such as the pyrazole (16) or aminothiadiazole (17) resulted in some of the most potent compounds. However, the poor solubility for these analogues led to low Cmax and poor oral exposure in mice. Only those compounds displaying blood- and liver-schizont activity (